Transient activation of c-MYC expression is critical for efficient platelet generation from human induced pluripotent stem cells

被引:241
|
作者
Takayama, Naoya [1 ]
Nishimura, Satoshi [3 ,4 ,5 ]
Nakamura, Sou [1 ]
Shimizu, Takafumi [2 ]
Ohnishi, Ryoko [1 ]
Endo, Hiroshi [1 ,2 ]
Yamaguchi, Tomoyuki [2 ]
Otsu, Makoto [2 ]
Nishimura, Ken [5 ,6 ]
Nakanishi, Mahito [6 ]
Sawaguchi, Akira [7 ]
Nagai, Ryozo [3 ,4 ]
Takahashi, Kazutoshi [8 ]
Yamanaka, Shinya [8 ]
Nakauchi, Hiromitsu [2 ]
Eto, Koji [1 ]
机构
[1] Univ Tokyo, Stem Cell Bank, Tokyo 1130033, Japan
[2] Univ Tokyo, Div Stem Cell Therapy, Ctr Stem Cell Biol & Regenerat Med, Inst Med Sci, Tokyo 1130033, Japan
[3] Univ Tokyo, Dept Cardiovasc Med, Tokyo 1130033, Japan
[4] Univ Tokyo, Translat Syst Biol & Med Initiat, Tokyo 1130033, Japan
[5] Japan Sci & Technol Agcy, PRESTO, Tokyo 1028666, Japan
[6] Natl Inst Adv Ind Sci & Technol, Gene Funct Res Ctr, Tsukuba 3058562, Japan
[7] Miyazaki Univ, Fac Med, Dept Anat, Miyazaki 8891692, Japan
[8] Kyoto Univ, Ctr iPS Res & Applicat, Kyoto 6068507, Japan
来源
JOURNAL OF EXPERIMENTAL MEDICINE | 2010年 / 207卷 / 13期
关键词
IN-VITRO; DIFFERENTIATION; MOUSE; MEGAKARYOCYTES; INFLAMMATION; FIBROBLASTS; BIOGENESIS; INDUCTION; PATHWAY; COMPLEX;
D O I
10.1084/jem.20100844
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Human (h) induced pluripotent stem cells (iPSCs) are a potentially abundant source of blood cells, but how best to select iPSC clones suitable for this purpose from among the many clones that can be simultaneously established from an identical source is not clear. Using an in vitro culture system yielding a hematopoietic niche that concentrates hematopoietic progenitors, we show that the pattern of c-MYC reactivation after reprogramming influences platelet generation from hiPSCs. During differentiation, reduction of c-MYC expression after initial reactivation of c-MYC expression in selected hiPSC clones was associated with more efficient in vitro generation of CD41a(+)CD42b(+) platelets. This effect was recapitulated in virus integration-free hiPSCs using a doxycycline-controlled c-MYC expression vector. In vivo imaging revealed that these CD42b(+) platelets were present in thrombi after laser-induced vessel wall injury. In contrast, sustained and excessive c-MYC expression in megakaryocytes was accompanied by increased p14 (ARF) and p16 (INK4A) expression, decreased GATA1 expression, and impaired production of functional platelets. These findings suggest that the pattern of c-MYC expression, particularly its later decline, is key to producing functional platelets from selected iPSC clones.
引用
收藏
页码:2817 / 2830
页数:14
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